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20
DISORDERS OF BILIRUBIN
METABOLISM
NAMITA ROY CHOWDHURY
IRWIN M. ARIAS
ALLAN W. WOLKOFF
JAYANTA ROY CHOWDHURY
FORMATION OF BILIRUBIN 292
Sources of Bilirubin 292
Enzymatic Mechanism of Bilirubin Formation 292
Quantification of Bilirubin Production 292
Inhibition of Bilirubin Production 293
CHEMISTRY OF BILIRUBIN 293
Absorption Spectra and Fluorescence 293
Effect of Light 293
QUANTIFICATION OF BILIRUBIN IN
BODY FLUIDS 293
TOXICITY OF BILIRUBIN 294
DISPOSITION OF BILIRUBIN 294
Bilirubin Transport in Plasma 294
Bilirubin Uptake by the Hepatocytes 295
Hepatocellular Storage of Bilirubin 295
Conjugation of Bilirubin 296
Canalicular Excretion of Conjugated Bilirubin 296
Bilirubin is the end product of degradation of the heme
moiety of hemoproteins. Hemoglobin, derived from senescent erythrocytes, is the major source of bilirubin. Significant fractions are also derived from other hemoproteins of
liver and other organs. Historically, hyperbilirubinemia has
attracted the attention of clinicians as a marker of liver dysN. Roy Chowdhury: Department of Medicine and Molecular Genetics,
Albert Einstein College of Medicine, Bronx, New York 10461.
I. M. Arias: Departments of Physiology and Medicine, Tufts University
School of Medicine, Boston, Massachusetts 02111.
A. W. Wolkoff: Departments of Medicine and Anatomy and Structural
Biology, Albert Einstein College of Medicine, Bronx, New York 10461-1602.
J. Roy Chowdhury: Department of Medicine and Molecular Genetics,
Albert Einstein College of Medicine Liver Center; Department of Medicine,
Jack D. Weiler Hospital of Albert Einstein College of Medicine, Bronx, New
York 10461.
Fate of Bilirubin in the Gastrointestinal Tract 296
Alternative Routes of Bilirubin Elimination 297
Antioxidant Property of Bilirubin 297
DISORDERS OF BILIRUBIN METABOLISM
RESULTING IN UNCONJUGATED
HYPERBILIRUBINEMIA 297
Neonatal Jaundice 298
Bilirubin Overproduction 298
Crigler–Najjar Syndrome Type 1 298
Crigler–Najjar Syndrome Type 2 (Arias Syndrome) 301
Gilbert Syndrome 302
DISORDERS OF BILIRUBIN METABOLISM THAT
RESULT IN PREDOMINANTLY CONJUGATED
HYPERBILIRUBINEMIA 303
Dubin–Johnson Syndrome 303
Rotor Syndrome 305
Progressive Familial Intrahepatic Cholestasis Syndromes 305
Alagille Syndrome 305
function. Subsequently, the studies of bilirubin chemistry,
synthesis, transport, metabolism, distribution, and excretion have provided important insights into the transport,
metabolism, and excretion of biologically important
organic anions, particularly those with limited aqueous solubility.
Bilirubin is potentially toxic, but is normally rendered
harmless by tight binding to albumin, and rapid detoxification and excretion by the liver. Patients with very high levels of unconjugated hyperbilirubinemia are at risk for
bilirubin encephalopathy (kernicterus). Kernicterus is
found in some cases of severe neonatal jaundice and in
inherited disorders associated with severe unconjugated
hyperbilirubinemia. This chapter provides a brief review of
bilirubin metabolism and its inherited disorders.
292
Chapter 20
FORMATION OF BILIRUBIN
Sources of Bilirubin
The breakdown of hemoglobin, other hemoproteins, and
free heme generates 250 to 400 mg of bilirubin daily in
humans, approximately 80% of which is derived from the
hemoglobin (1). Intravenously administered radiolabeled
porphyrin precursors (glycine or δ-aminolevulinic acid) are
incorporated into bile pigments in two peaks (2). The
“early-labeled” peak appears within 72 hours. The initial
component of this peak is derived mainly from hepatic
hemoproteins such as cytochromes, catalase, peroxidase,
and tryptophan pyrrolase, and a small, rapidly turning over
pool of free heme. The slower phase of the early-labeled
peak is derived from both erythroid and nonerythroid
sources, and is enhanced in conditions associated with
“ineffective erythropoiesis,” e.g., congenital dyserythropoietic anemias, megaloblastic anemias, iron-deficiency anemia, erythropoietic porphyria and lead poisoning (3), and
in accelerated erythropoiesis (4). A “late-labeled” peak
appears at approximately 110 days in humans and 50 days
in rats, and represents the contribution from the hemoglobin of senescent erythrocytes.
Enzymatic Mechanism of Bilirubin
Formation
Heme (ferroprotoporphyrin IX) (Fig. 20.1) is cleaved by
selective oxidation of the α-methene bridge, catalyzed by
microsomal heme oxygenase. This reaction requires three
molecules of O2 and a reducing agent, such as reduced
FIGURE 20.1. Mechanism of heme ring opening and subsequent reduction of biliverdin to bilirubin.
nicotinamide adenine dinucleotide phosphate (NADPH),
and results in the formation of the linear tetrapyrrole,
biliverdin, and 1 mol of CO. The iron molecule is released
(5). Three forms of heme oxygenase have been identified
(6). Heme oxygenase 1 is ubiquitous and is a major
inducible stress-related protein. Heme oxygenase 1 synthesis is upregulated by heme (7). In contrast, heme oxygenase
2 is a constitutive protein, expressed mainly in the brain
and the testis. Heme oxygenase 3 has very low catalytic
activity and may function mainly as a heme-binding protein. The products of heme oxygenase, biliverdin (which is
subsequently reduced to bilirubin), and CO have significant physiologic effects. CO, a potent vasodilator, regulates
the vascular tone in the liver and in other organs, such as
the heart, under conditions of stress. Biliverdin and bilirubin are potent antioxidants, and may protect tissues under
oxidative stress (6,8).
In most mammals, biliverdin is reduced to bilirubin by
the action of biliverdin reductases. The physiologic advantage of this process is not clear, because bilirubin requires
energy-consuming metabolic modification for excretion in
bile. The stronger antioxidant activity of bilirubin may be
particularly important during the neonatal period, when
concentrations of other antioxidants are low in body fluids.
Biliverdin reductases are cytosolic enzymes that require
reduced nicotinamide adenine dinucleotide (NADH) or
NADPH for activity (9).
Quantification of Bilirubin Production
At a steady-state condition of blood hemoglobin level, the
rate of bilirubin production equals the rate of heme synthesis. Therefore, the heme synthesis rate can be estimated
from the rate of bilirubin production. In humans, bilirubin
production can be quantified from the turnover of intravenously administered radioisotopically labeled bilirubin.
Plasma bilirubin clearance (the fraction of plasma from
which bilirubin is irreversibly extracted) is proportional to
the reciprocal of the area under the radiobilirubin disappearance curve (10). Bilirubin removal is calculated from
the product of plasma bilirubin concentration and clearance. When plasma bilirubin concentrations remain constant, removal of bilirubin equals the amount of newly synthesized bilirubin entering the plasma pool. Alternatively,
bilirubin formation can also be quantified from carbon
monoxide production. Following rebreathing in a closed
system, CO production is calculated from the CO concentration in the breathing chamber and/or the increment in
blood carboxyhemoglobin saturation (11). CO production
exceeds plasma bilirubin turnover by 12% to 18%, because
a fraction of bilirubin produced in the liver is excreted into
bile without appearing in serum. A small fraction of the CO
may be formed by intestinal bacteria (12).
Disorders of Bilirubin Metabolism
Inhibition of Bilirubin Production
Nonmetabolized “dead-end” inhibitors of heme oxygenase,
such as tin-protoporphyrin or tin-mesoporphyrin, inhibit
heme oxygenase activity (13). Injection of tin-mesoporphyrin
in neonates reduces serum bilirubin levels by 76% (14).
CHEMISTRY OF BILIRUBIN
The systemic name of bilirubin IXα is 1,8-dioxo-1,3,6,7tetramethyl-2,8-divinylbiladiene-a,c-dipropionic acid (15,
16). The linear tetrapyrrole structure of bilirubin was solved
by Fischer and Plieninger (17). X-ray diffraction studies of
crystalline bilirubin has revealed that the propionic acid
side chains of bilirubin are internally hydrogen-bonded to
the pyrrolic and lactam sites on the opposite half of the
molecule (18). The molecule takes the form of a “ridge tile”
in which the two dipyrrolic halves of the molecule lie in two
different planes with an interplanar angle of 98 to 100
degrees (Fig. 20.2). The integrity of the hydrogen-bonded
structure requires the interpyrrolic bridges at the 5 and 15
position of bilirubin to be in trans- or Z configuration. The
hydrogen-bonded structure of bilirubin explains many of
its physicochemical properties. As both the carboxylic
groups, all four NH groups, and the two lactam oxygens are
293
engaged by hydrogen bonding, bilirubin is insoluble in
water. The hydrogen bonds “bury” the central methene
bridge, so that the molecule reacts very slowly with diazo
reagents. In vivo, the hydrogen bonds are disrupted by
esterification of the propionic acid carboxyl group with glucuronic acid (see below). Because of this disruption, conjugated bilirubin reacts rapidly with diazo reagents (“direct”
van den Bergh reaction). Addition of methanol, ethanol, 6
M urea, or dimethyl sulfoxide to plasma disrupts the hydrogen bonds of bilirubin, rendering the molecule water soluble and making the central methene bridge readily accessible, so that both conjugated and unconjugated bilirubin
react rapidly with diazo reagents (“total” van den Bergh
reaction) (19).
Absorption Spectra and Fluorescence
The main absorption band of unconjugated bilirubin IXα
is at 450 to 474 nm in most organic solvents. Although
pure bilirubin does not fluoresce, when dissolved in detergents, albumin solution, or alkaline methanol, an intense
fluorescence is observed at 510 to 530 nm. Fluorescence
determination has been utilized for rapid quantification of
blood bilirubin concentrations and the unsaturated bilirubin-binding capacity of albumin (see below).
Effect of Light
The “Z” (trans) configuration of the 5 and/or 15 carbon
bridges of bilirubin is changed to the “E” (cis) configuration upon exposure to light. The resulting ZE, EZ, or EE
isomers lack internal hydrogen bonds, are more polar than
bilirubin IXα-ZZ, and can be excreted in bile without conjugation (20). The vinyl substituent in the endovinyl half of
bilirubin IXα-EZ is slowly cyclized with the methyl substituent on the internal pyrrole ring, forming the stable
structural isomer, E-cyclobilirubin, which is quantitatively
important during phototherapy for neonatal jaundice (21).
In the presence of light and oxygen, a fraction of the bilirubin molecules is also converted to colorless fragments (22).
A small amount of biliverdin is also formed (22).
QUANTIFICATION OF BILIRUBIN IN BODY
FLUIDS
FIGURE 20.2. X-ray crystallographic structure of bilirubin showing a ridge-tile configuration caused by internal hydrogen bonding of the propionic acid carboxyls to the amino groups and the
lactam oxygen of the pyrrolenone rings of the opposite half of
the molecule. The bonds between the pyrrolenone rings A and B
and C and D are in the Z (trans) configuration.
Bile pigments are quantified as native or derivatized
tetrapyrroles, or after conversion to azoderivatives. Total
bilirubin can also be quantified indirectly by quantification
of the intensity of yellow discoloration of the skin. Conversion to azodipyrroles by reaction with diazo reagents is used
commonly for determination of serum bilirubin levels for
clinical purposes. Electrophilic attack on the central bridge
splits bilirubin into two diazotized azodipyrrole molecules.
294
Chapter 20
As discussed above, conjugated bilirubin reacts rapidly in this
system (direct fraction). In the presence of accelerators, both
unconjugated and conjugated bilirubin react rapidly (total
bilirubin). Unconjugated bilirubin (the “indirect” fraction) is
calculated by subtracting the direct fraction from total bilirubin. As 10% to 15% of unconjugated bilirubin may give the
direct diazo reaction, this method slightly overestimates conjugated bilirubin. The irreversibly albumin-bound fraction of
serum bilirubin, which is formed in the serum of patients
with prolonged conjugated hyperbilirubinemia, also exhibits
direct diazo reaction (23). For more accurate quantification
and for separating the different sugar conjugates, the intact
bilirubin tetrapyrroles can be separated by thin-layer or highperformance liquid chromatography (24–26). Bilirubin
mono- and diconjugates can be converted to methyl esters by
alkaline methanolysis prior to separation (27), but because
the sugar groups are cleaved off, this method does not permit
identification of specific conjugates.
For repeated bilirubin measurements, particularly in jaundiced infants, special clinical methods have been devised.
Measurement of the yellow color of the skin by analysis of
reflected light provides a noninvasive approach for estimating
serum bilirubin (28), which has been verified in a large study
(29). Two slide tests are available for determination of total
bilirubin, and the unconjugated, conjugated, and irreversibly
protein-bound fractions. Fluorescence characteristics of bilirubin have been utilized for determining total bilirubin, albumin-bound bilirubin, and reserve bilirubin-binding capacity
from as little as 0.1 mL of whole blood (30).
About 4% of bilirubin in normal plasma is conjugated, but
the clinical diazo-based methods overexpress this fraction (see
above). In hemolytic jaundice, there is a proportionate
increase of plasma unconjugated and conjugated bilirubin. In
contrast, in inherited disorders of bilirubin conjugation, the
conjugated bilirubin is absent or reduced in proportion. In
biliary obstruction or hepatocellular diseases, both conjugated
and unconjugated bilirubin accumulate in plasma. Bilirubin is
present in exudates and other albumin containing body fluids
and binds to the elastic tissue of skin and sclera. Heme in subcutaneous hematomas is sequentially converted to biliverdin
and bilirubin, resulting in a transition from green to yellow
discoloration. Because of tight binding to albumin, unconjugated bilirubin is not excreted in urine in the absence of albuminuria, but conjugated bilirubin, which is less strongly
bound to albumin, appears in urine. Bilirubin is present in
normal human bile predominantly as diglucuronide, with
unconjugated bilirubin accounting for only 1% to 4% of the
pigments (see below).
TOXICITY OF BILIRUBIN
The toxic effect of bilirubin on the brain of neonates has
been known since antiquity. Yellow discoloration of basal
ganglia is termed kernicterus. Bilirubin exhibits a wide
range of toxic effects in cell culture systems and in cell
homogenates. Bilirubin inhibits DNA synthesis in a mouse
neuroblastoma cell line (31), and uncouples oxidative phosphorylation and inhibits adenosine triphosphatase (ATPase)
activity of brain mitochondria (32). In mutant rats (Gunn
strain) with congenital nonhemolytic hyperbilirubinemia
(see below), bilirubin inhibited RNA and protein synthesis,
and carbohydrate metabolism in brain (33). In a cell-free
system, bilirubin inhibited Ca2+-activated, phospholipiddependent, protein kinase (protein kinase C) activity and
3⬘,5⬘-cyclic adenosine monophosphate (cAMP)-dependent
protein kinase activity (34), which may be relevant in the
mechanism of its toxicity. Albumin binding inhibits toxic
effects of bilirubin, both in vitro and in vivo.
At serum unconjugated bilirubin concentrations over 20
mg/dL, newborn babies are at risk of kernicterus. However,
kernicterus can occur at lower concentrations (35). Serum
albumin concentrations, pH, and substances that compete for
albumin binding are important in the pathogenesis of bilirubin encephalopathy (36). The immaturity of the blood–brain
barrier in neonates is often held responsible for increased susceptibility of neonates to kernicterus. Tight junctions between
capillary endothelial cells and foot processes of astroglial cells
that restrict the exchange of water-soluble substances and proteins between blood and brain are the anatomic constituents
of the blood–brain barrier (37). In addition, specific transport
processes for ions, water, and nutrients from plasma to brain
may provide a functional blood–brain barrier. However, there
is little evidence to support the concept of immaturity of the
blood–brain barrier in the neonate. The opening of the
blood–brain barrier is expected to permit the entrance of albumin-bound bilirubin into the brain, which should not result
in increased bilirubin toxicity. The entry of the non–albuminbound (free) fraction of bilirubin into the brain is independent of the intactness of the blood–brain barrier. Damaged
and edematous brain may bind bilirubin avidly, and therefore
be unable to clear it rapidly, increasing the susceptibility to
bilirubin encephalopathy (38).
DISPOSITION OF BILIRUBIN
Hepatocellular disposition of bilirubin requires several specific
physiologic mechanisms, including transport to the hepatocytes from the major sites of production, efficient internalization into the hepatocyte, enzyme-catalyzed conjugation with
glucuronic acid, active transport into the bile canaliculus, and
degradation in the intestinal tract. These steps are summarized
in Fig. 20.3, and briefly discussed below.
Bilirubin Transport in Plasma
Bilirubin is tightly but reversibly bound to plasma albumin.
Albumin binding keeps bilirubin in solution and transports
the pigment to the liver. Unconjugated bilirubin is bound
Disorders of Bilirubin Metabolism
295
FIGURE 20.3. Summary of hepatic metabolism of bilirubin. Bilirubin is strongly bound to albumin in the circulation (1). At the sinusoidal surface of the hepatocyte, this complex dissociates,
and bilirubin enters hepatocytes by facilitated diffusion (2). This process is non-adenosine triphosphate (ATP)-dependent and bidirectional. Within the hepatocyte, bilirubin binds to a group of
cytosolic proteins, mainly to glutathione-S-transferases (GSTs) (3). GST binding inhibits the efflux
of bilirubin from the cell, thereby increasing the net uptake. A specific form of uridine diphosphoglucuronate glucuronosyltransferase (UGT) (BUGT, also termed UGT1A1), located in the
endoplasmic reticulum, catalyzes the transfer of the glucuronic acid moiety from UDP-glucuronic
acid (UDPGA) to bilirubin, forming bilirubin diglucuronide and monoglucuronide (4). Glucuronidation is necessary for efficient excretion of bilirubin in bile (5). Canalicular excretion of
bilirubin and other organic anions (except most bile acids) is primarily an energy-dependent
process, mediated by the ATP-utilizing transporter multidrug resistance-related protein (MRP2),
also termed canalicular multispecific organic anion transporter (cMOAT).
tightly to albumin and, therefore, is not excreted in urine,
except during albuminuria. Conjugated bilirubin is bound
less tightly to albumin, and the unbound fraction is
excreted in the urine. During prolonged conjugated hyperbilirubinemia, a fraction of the pigment becomes irreversibly bound to albumin. This fraction, termed deltabilirubin, is not excreted in the bile or urine and disappears
slowly, reflecting the long half-life of albumin (23).
Albumin binding protects against the toxic effects of
bilirubin. A small unbound fraction of bilirubin is thought
to be responsible for its toxicity (39). Normally, the molar
concentration of albumin (500 to 700 μmol/L) exceeds that
of bilirubin (3 to 17 μmol/L). However, during neonatal
jaundice, in patients with Crigler–Najjar syndrome, the
molar ratio of unconjugated bilirubin to albumin may
exceed 1. Reduction of serum albumin levels during inflammatory states, chronic malnutrition, or liver diseases may
accentuate bilirubin toxicity. Sulfonamides, antiinflammatory drugs, and cholecystographic contrast media displace
bilirubin competitively from albumin and increase the risk
of kernicterus in jaundiced infants (40). Binding of short
chain fatty acids to albumin causes conformational changes,
decreasing bilirubin binding.
Because of the pathophysiologic importance of the
unbound fraction of unconjugated bilirubin, ultrafiltration,
ultracentrifugation, gel chromatography, affinity chro-
matography on albumin agarose polymers, dialysis, and
electrophoresis have been used to separate free from bound
bilirubin. Unbound bilirubin is rapidly destroyed by treatment with H2O2 and horseradish peroxidase, as compared
with bound bilirubin. Binding of bilirubin to albumin
induces bilirubin fluorescence, and quenches the protein
fluorescence. This phenomenon has been utilized for differentiating free from albumin-bound bilirubin.
Bilirubin Uptake by the Hepatocytes
At the sinusoidal surface of the hepatocyte (Fig. 20.3), bilirubin dissociates from albumin and is taken up by the hepatocyte by facilitated diffusion. The transport requires the presence of inorganic anions, such as Cl−. A family of organic
anion transport proteins (oatp) has been identified. One oatp
isoform, oatp-1, mediates Na+-independent taurocholate
transport and is associated with HCO3− exchange (41). However, the role of oatp family of proteins in bilirubin transport
has not been directly established (see Chapter 7).
Hepatocellular Storage of Bilirubin
Within the hepatocyte, bilirubin is kept in solution by binding to cytosolic proteins, which were originally designated Y
and Z. The Y group of proteins, which constitute 5% of the
296
Chapter 20
liver cytosol, binds various drugs, hormones, organic anions,
a cortisol metabolite, and azo-dye carcinogens, and was
termed “ligandin” (42). Subsequently, ligandin was found to
be a family of proteins, identical to the α class of glutathioneS-transferases (GST) in the rat liver (43). There are corresponding proteins in human hepatocytes as well. Binding to
GSTs increases the net uptake of bilirubin by reducing efflux
from the hepatocyte (Fig. 20.3). GST binding may inhibit
the toxicity of bilirubin by preventing its nonspecific diffusion into specific subcellular compartments. For example,
binding to GSTs prevents the inhibition of mitochondrial
respiration by bilirubin in vitro (44).
Conjugation of Bilirubin
Conversion to bilirubin diglucuronide or monoglucuronide
by esterification of both or one of the propionic acid carboxyl
groups is critical for efficient excretion of bilirubin across the
bile canaliculus (Fig. 20.3). Bilirubin diglucuronide accounts
for about 80% of pigments excreted in normal bile (24–26).
Bilirubin monoglucuronide constitutes about 10% of the
pigments, but in states of partial deficiency of hepatic bilirubin glucuronidation the proportion of bilirubin monoglucuronide increases (see Crigler–Najjar Syndrome Type 2 and
Gilbert Syndrome, below). Smaller amounts of glucosyl and
xylosyl conjugates are also found.
Bilirubin-Uridine Diphosphoglucuronate
Glucuronosyltransferase
Glucuronidation of bilirubin is catalyzed by a specific isoform of uridine diphosphoglucuronate glucuronosyltransferase (UGT). UGTs comprise a family of enzymes that are
integral components of the endoplasmic reticulum of various cell types (45). UGTs mediate the conversion of a wide
variety of exogenous and endogenous toxic metabolites to
less bioreactive, polar compounds that are readily eliminated in bile or urine. Based on the degree of homology of
the messenger RNA (mRNA) sequences, UGTs have been
categorized into several families and subfamilies (46). Only
one of these UGT isoforms, currently termed UGT1A1,
contributes significantly to bilirubin glucuronidation (47).
The gene that expresses bilirubin-UGT (UGT1A1) is
termed UGT1A (48). The UGT1A locus contains four consecutive exons (exons 2 to 5) at the 3⬘ end that are used in
all mRNAs expressed from this locus, and encode the identical upidine diphospho (UDP)-glucuronic acid-binding
carboxy-terminal domain of the UGT isoforms (Fig. 20.4).
Upstream to these four common-region exons is a series of
unique exons, each preceded by a separate promoter, only
one of which is utilized in specific UGT mRNAs. The
unique exon encodes the variable aglycone-binding N-terminal domain of individual UGT isoforms. Depending on
which promoter is used, transcripts of various lengths are
generated. The unique exon, located at the 5⬘ end of the
transcript, is spliced to exon 2, and the intervening
sequence is spliced out. Within the UGT1A locus, genes
encoding individual isoforms are named after the unique
exon that is utilized in the specific mRNA. Bilirubin-UGT
mRNA, which consists of the first unique region exon of
the UGT1A locus (plus exons 2 to 5), is named UGT1A1
according to this terminology.
The presence of a separate promoter upstream to each
unique region exon (Fig. 20.4) permits differential expression of individual UGT isoforms during development (49)
and enzyme induction (50). UGT1A1 develops after birth
(49) and is induced by phenobarbital and clofibrate (51).
Treatment of rats with triiodothyronine markedly reduces
UGT activity toward bilirubin, whereas the activity toward
4-nitrophenol is increased (50).
Canalicular Excretion of Conjugated
Bilirubin (See Chapters 24, 25, and 26)
Conjugated bilirubin is excreted across the bile canaliculus against a concentration gradient, which can be as high
as 150-fold. The energy for the uphill transport of bilirubin is provided by an adenosine triphosphate (ATP)dependent system in the canalicular membranes that is
specific for non–bile-acid organic anions, including bilirubin and other glucuronides, and glutathione conjugates
(52,53). A canalicular membrane protein, termed canalicular multispecific organic anion transporter (cMOAT) or
multidrug resistance-related protein (MRP2) (54), mediates the ATP-dependent canalicular organic anion transport.
Fate of Bilirubin in the Gastrointestinal
Tract
Conjugated bilirubin is not substantially absorbed from
the gastrointestinal tract. When there is enhanced excretion of unconjugated bilirubin into the intestine, e.g.,
during phototherapy for neonatal jaundice or Crigler–
Najjar syndrome, absorption of unconjugated bilirubin
from the intestine may be clinically significant (55). Milk
inhibits intestinal absorption of unconjugated bilirubin,
but such inhibition is less with human milk than with
infant milk formula. Intestinal bacteria degrade bilirubin
into a series of urobilinogen and related products (56).
Most of the urobilinogen reabsorbed from the intestine is
excreted in bile, but a small fraction is excreted in urine.
Absence of urobilinogen in stool and urine indicates complete obstruction of the bile duct. In liver disease and
states of increased bilirubin production, urinary urobilinogen excretion is increased. Urobilinogen is colorless;
its oxidation product, urobilin, contributes to the color of
normal urine and stool.
Disorders of Bilirubin Metabolism
297
FIGURE 20.4. Schematic representation of the human UGT1A locus, located at 2q37. This locus
comprises a number of genes of the UGT1A family that include bilirubin-UGT. Exons 2, 3, 4, and 5,
located at the 3⬘ end of UGT1A, encode the identical carboxyl terminal domains of all UGT1A isoforms expressed from this locus. Upstream to these “common region” exons are a series of “unique
exons” (exons 1A1 through 1A12), each of which encodes the variable amino terminal domain of
a different UGT1A isoform. Each unique region exon is preceded by a separate promoter region
(arrows), permitting independent regulation of gene expression. Transcription may start from any
of the promoters, producing transcripts of varying lengths, two examples of which are shown in
the figure. The unique exon located at the 5⬘ end of the primary transcript is spliced to the 5⬘ end
of exon 2, and other unique region exons present in the transcript (shown in dotted lines) are
spliced out. Genes belonging to the UGT1A locus are named according the unique exon utilized in
the processed mRNA. Thus, when the transcription starts at exon 1A4 (upper transcript in the figure), the mRNA for UGT1A4 is generated after splicing. This gene, which consists of exon 1A4 plus
the common region exons 2 to 5, is termed UGT1A4, and the expressed enzyme is termed UGT1A4.
Similarly, if the transcription starts at exon 1A1 (lower transcript in the figure), an mRNA consisting of exon 1A1 plus exons 2 to 5 is generated. According to the current system of terminology, this
gene is named UGT1A1, and the expressed isoform is termed UGT1A1. UGT1A1 is the only isoform
that contributes significantly to bilirubin glucuronidation in humans. This structure predicts that
disorders of bilirubin glucuronidation resulting from genetic lesions within exon 1A1 should affect
UGT activity toward bilirubin, but other UGT1A isoforms should be normal. In contrast, mutations
of exons 2 to 5 should affect all isoforms of the UGT1A family.
Alternative Routes of Bilirubin
Elimination
In the absence of bilirubin glucuronidation, a small fraction of
bilirubin is excreted as hydroxylated products. Induction of a
specific isoform of microsomal P-450s by administration of
2,3,7,8-tetrachlorodibenzo-p-dioxin (TCDD) in UGT1A1deficient Gunn rats resulted in a sevenfold increase in the fractional turnover of bilirubin and reduction of the bilirubin
pool (57). A mitochondrial bilirubin oxidase in liver (58) and
other tissues may catalyze oxidative degradation of bilirubin.
During intrahepatic or extrahepatic cholestasis, the
plasma conjugated bilirubin concentrations increase. In
total biliary obstruction, renal excretion becomes the major
pathway of bilirubin excretion. Renal excretion of conjugated bilirubin depends on glomerular filtration of the
non–protein-bound fraction of conjugated bilirubin.
Antioxidant Property of Bilirubin
Although bilirubin has been thought of conventionally as a
waste product with little utility, antioxidant activity of
bilirubin may serve an important tissue protective role.
Both unconjugated (59) and conjugated (60) bilirubin
inhibit lipid peroxidation. The tissue cytoprotective role of
heme oxygenase in various tissues may be mediated by
biliverdin and bilirubin.
DISORDERS OF BILIRUBIN METABOLISM
RESULTING IN UNCONJUGATED
HYPERBILIRUBINEMIA
Hepatic transport of bilirubin involves four distinct but
probably interrelated stages: (a) uptake from the circula-
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Chapter 20
tion; (b) intracellular binding or storage; (c) conjugation,
largely with glucuronic acid; and (d) biliary excretion.
Abnormalities in any of these processes may result in hyperbilirubinemia. Complex clinical disorders, such as hepatitis
or cirrhosis, may affect multiple processes. In several inherited disorders, the transfer of bilirubin from blood to bile is
disrupted at a specific step. Study of these disorders has permitted better understanding of bilirubin metabolism in
health and disease. Each disorder is characterized by varied
degrees of hyperbilirubinemia of the unconjugated or conjugated type.
Neonatal Jaundice
By adult standards, every newborn baby has increased
serum bilirubin levels, and about half of all neonates
become clinically jaundiced during the first 5 days of life.
Serum bilirubin is predominantly unconjugated. Exaggeration of this “physiologic jaundice” exposes the baby to the
risk of kernicterus (see Toxicity of Bilirubin, above). In 16%
of newborns, maximal serum bilirubin concentrations equal
or exceed 10 mg/dL, and in 5% serum bilirubin levels are
above 15 mg/dL. In the normal full-term neonates, serum
bilirubin peaks at approximately 72 hours and subsequently
declines to normal adult levels in 7 to 10 days. Physiologic
jaundice of the newborn results from a combination of
increased bilirubin production and immaturity of the
bilirubin disposal mechanisms of the liver. Bilirubin production rate is high in newborns, because of the increased
early-labeled peak from erythroid and nonerythroid
sources, and decreased erythrocyte half-life (61). Net
hepatic bilirubin uptake is low in neonates because of low
hepatocellular ligandin levels (62). Delayed closure of the
ductus venosus may permit the bilirubin-rich portal blood
to bypass the liver. Low caloric intake may also reduce
hepatic bilirubin clearance. UGT activity toward bilirubin
is low in the liver of the newborn and takes about 10 days
to mature to adult levels (63). Deficiency of UGT activity
may be prolonged and exaggerated in some inherited disorders due to inhibitory factor(s) in maternal milk or serum
(see Gilbert syndrome, below). A variant TATAA element
within the promoter region of UGT1A1 has been found to
be associated with Gilbert syndrome (64) (see Gilbert syndrome, below). Presence of this variant promoter reduces
the expression of bilirubin-UGT (UGT1A1) and may
accentuate and prolong neonatal jaundice (65).
Plasma bilirubin concentrations tend to be higher in
breast-fed infants than in formula-fed babies. The hyperbilirubinemia resolves on discontinuation of breast-feeding,
and kernicterus occurs only rarely (66). Maternal milk
jaundice is associated with an inhibitor of UGT activity in
maternal milk but not maternal serum (67). Free fatty acids
resulting from the digestion of fat by lipase secreted in the
milk of some women are thought to inhibit hepatic bilirubin-UGT activity (68). Intestinal absorption of unconju-
gated bilirubin is high in neonates. Bilirubin absorption
may be higher in breast-fed infants than in formula-fed
babies.
Inhibitory factors present in the plasma of some mothers
may delay the maturation of bilirubin-UGT (69). Peak
serum bilirubin concentrations of 8.9 to 65 mg/dL are
reached within 7 days. This condition, termed LuceyDriscoll syndrome, is distinguished from maternal milk
jaundice by earlier onset of hyperbilirubinemia, a more
severe and protracted course, and occasional kernicterus.
In the great majority of cases, neonatal hyperbilirubinemia is innocuous. But vigilance is needed for the occasional
case in which severe neonatal jaundice can expose the newborn to the risk of kernicterus. Although plasma bilirubin
levels of 20 mg/dL or higher are considered dangerous,
bilirubin encephalopathy may occur at lower concentrations (see Toxicity of Bilirubin, above). Phototherapy is the
most common treatment used. In severe cases exchange
transfusion is employed to reduce serum bilirubin levels
rapidly. Inhibition of heme oxygenase activity by the
administration of tin-mesoporphyrin at birth has been
shown to prevent the development of significant levels of
neonatal jaundice, thereby abrogating the need for phototherapy or exchange transfusion.
Bilirubin Overproduction
Bilirubin overproduction results in unconjugated hyperbilirubinemia, which rarely exceeds 3 to 4 mg/dL in the
absence of hepatobiliary dysfunction. Bilirubin overproduction occurs commonly in hemolytic conditions and during
resolution of large hematomas. Ineffective erythropoiesis
occurs in thalassemia, pernicious anemia, and some rare
hereditary anemias, termed congenital dyserythropoietic anemias (70). In addition to unconjugated bilirubin, a small
amount of conjugated bilirubin may accumulate in the
serum (~4% of total bilirubin), probably because of diffusion
out of the hepatocyte. This does not necessarily indicate that
the rate of bilirubin production has exceeded the hepatic
excretory transport maximum for conjugated bilirubin.
Crigler–Najjar Syndrome Type 1
Crigler–Najjar syndrome type I is a rare disorder, characterized by severe lifelong nonhemolytic unconjugated hyperbilirubinemia (71) (Table 20.1). Hepatic bilirubin-UGT
activity is absent or nearly so. Without treatment, the majority of patients used to die of kernicterus during the first 18
months of life. Exceptional patients survived beyond
puberty, but succumbed to bilirubin encephalopathy in
young adult life (72,73). With the routine use of phototherapy and intermittent plasmapheresis during crises, survival
until puberty is usual, but the risk of bilirubin encephalopathy increases at this age (74). Orthotopic or auxiliary liver
transplantation cures the disease.
Disorders of Bilirubin Metabolism
299
TABLE 20.1. CHARACTERISTICS OF INHERITED UNCONJUGATED HYPERBILIRUBINEMIA
Crigler–Najjar
Syndrome Type 1
Liver function tests other
than serum bilirubin
and liver histology
Serum bilirubin
concentrations
Pigments excreted in bile
Hepatic bilirubin-UGT
activity
Effect of phenobarbital
administration
Inheritance
Molecular basis
Prevalence
Prognosis
Animal model
Crigler–Najjar
Syndrome Type 2
Gilbert Syndrome
Normal
Normal
Normal
20–50 mg/dL
(340–850 μM)
Small amounts of
unconjugated bilirubin
and only traces of
bilirubin glucuronides
Virtually absent
7–20 mg/dL
(120–340 μM)
Reduced proportion
of bilirubin
diglucuronide
Normal to 5 mg/dL (<85 μM)
Markedly reduced
but detectable
Reduction of serum
bilirubin levels
by >25%
Autosomal recessive
Point mutations
within the coding
region of UGT1A1
Rare (<1:1,000,000)
Reduced to about 30% of normal
No significant reduction
of serum bilirubin levels
Autosomal recessive
Genetic lesions within the
coding region or at
splice sites of UGT1A1
Rare (<1:1,000,000)
Kernicterus, unless vigorously
treated; currently, liver
transplantation is the
only curative treatment
Gunn rat
Reduced proportion of bilirubin diglucuronide
Normalization of serum bilirubin
Autosomal recessive
Insertion of a TA dinucleotide within the TATAA
element of UGT1A1a
Kernicterus is
uncommon, but
has been reported
Phenotype in ~4% of the population; among
Caucasians and Africans, ~9% are homozygous
for the genotype (less common in Japan)
No encephalopathy; increased intensity of
neonatal jaundice; toxicity of some drugs
may be increased
—
Bolivian subpopulation of squirrel monkeys
aSome
mutations of the coding region of UGT1A1 may be associated with serum bilirubin levels that overlap with the
range seen in Gilbert syndrome (Table 20.3).
UGT, uridine-diphosphoglucuronate glucuronosyl-transferase.
Laboratory test results in Crigler–Najjar syndrome type
1 are normal except for the serum bilirubin levels, which are
usually 20 to 25 mg/dL, but may increase during intercurrent illness to as high as 50 mg/dL (75). Serum bilirubin is
unconjugated and there is no bilirubinuria. There is no evidence of hemolysis. As the canalicular excretion process is
normal, oral cholecystography visualizes the gallbladder.
There is an increased incidence of pigment gallstones, probably because of increased concentrations of unconjugated
bilirubin in bile, resulting from phototherapy. Liver histology is normal except for the presence of “pigment plugs” in
bile canaliculi.
As UGT1A1 (bilirubin-UGT1) is the only isoform that
contributes significantly to bilirubin metabolism (47),
genetic lesions within the coding region of the UGT1A1
gene can abolish hepatic bilirubin glucuronidation, causing
Crigler–Najjar syndrome type 1. Since the initial description of the molecular basis of Crigler–Najjar syndrome in
1992 (48,76) numerous mutations, deletions, and insertions in any of the five exons of UGT1A1 have been shown
to cause the disease (77–89) (Table 20.2). In addition to
exonic lesions, mutations of the splice donor or splice
acceptor sites within the intronic sequences can cause inappropriate splicing of the transcript, resulting in the loss of
UGT1A1 activity. These molecular lesions have been
reviewed recently (90). As in all rare recessively inherited
disorders, known or unknown consanguinity is common,
but not always found (91). Crigler–Najjar syndrome is
found in all races. As many different mutations can cause
the disease, no single mutation is common in any race. An
exception to this is found among the Amish and Mennonite communities of Pennsylvania (92), where the disease is
relatively common and all patients have the same mutation,
reflecting a strong founder effect. In patients with genetic
lesions within the unique exon 1, only UGT1A1 activity is
abnormal, but when the mutation affects one of the common region exons (exons 2 to 5), all UGT1A group of isoforms are expected to be abnormal.
The differential diagnosis includes Crigler–Najjar syndrome type 2, with or without coexisting hemolysis.
Although serum bilirubin levels are relatively lower in
Crigler–Najjar syndrome type 2, the ranges overlap in the
two disorders. In most cases of Crigler–Najjar syndrome type
2, the serum bilirubin concentrations are reduced by more
than 25% after phenobarbital administration (60 to 120 mg
for 14 days), which differentiates it from Crigler–Najjar syndrome type 1 (75). Chromatographic analysis of pigments in
bile collected from the duodenum through a perorally placed
duodenal catheter or an upper gastrointestinal endoscope
provides rapid differentiation of the two conditions. In
300
Chapter 20
TABLE 20.2. GENETIC LESIONS OF UGT1A1 THAT ABOLISH BILIRUBIN–UGT
ACTIVITY (CRIGLER–NAJJAR SYNDROME TYPE 1)
Site of Lesion
Nucleic Acid Alteration
Predicted Mutation of UGT1A1
Activity
Reference
79
80
81
82
81–83
83
83
76,83,84
85
86
83
84
78,83
84,87
77
84
88
89
76,83,84
76,83,84
84
79
86
77,83,87
84
79
84
84
Exon 1
Exon 1
Exon 1
Del C,T at nt 120,121, respectively
Ins 4 bp after codon 80
Ins T after codon 158/del codon 170
Truncated (frameshift)
Truncation (frameshift)
Truncated (frameshift)/del of phenylalanine
Inactive
Inactive
Inactive/inactive
Exon 1
Exon 1/exon 2
Exon 1
Exon 1/exon 3
Exon 1
Intron 1
Exon 2
Exon 2/exon 4
Exon 2
Exon 2
Exon 2
Exon 3/exon 4
Exon 3
Exon 3
Exon 3
Exon 3/exon 4
Exon 3
Exon 3/exon 4
Intron 3/exon 1
Exon 4
Exon 4
Exon 4
Exon 4
Exon 4/exon 5
Del of codon 170
T529C/del nt 879–892
G826T
A835T/C1069T
C840A
Splice donor, G→C
Skipping of exon 2
C872T/A1282G
T880A and del 881–893
G923A
C991T
G1005A/G1102A
nt: C1006T
C1021T
C1069T
C1069T/G1201C
A1070G
C1081T/CC1159,1160GT
Splice acceptor site, A→G/nt C145T
C1124T
C1143G
CC1159,1160GT
G1201C
G1201C/A1308T
Del phenylalanine
C177R/truncated (frameshift)
G276R
B279Y/Q357X
C280X
Truncated
Truncated
A291V/K426E
Truncated (frameshift)
G308E
Q331X
W335X/A368T
R336W/N
R341X
Q357X
Q357X/A401P
Q357R
Q361X/P387R
Truncated protein/Q49X
S376F
S381R
P387R
A401P
A401P/K437X
Inactive
Inactive/inactive
Inactive
ND/inactive
Inactive
Inactive
Inactive
Inactive
Inactive
Inactive
Inactive
Inactive
Inactive
Inactive
Inactive
Inactive
Inactive
Inactive/inactive
Inactive
Inactive
Inactive
Inactive
Inactive
Inactive
bp, base pair; nt, nucleotide; del, deletion; ins, insertion; N, normal; ND, not determined. Note: A slash separating two
mutations indicates that the patient was a compound heterozygote for two different mutations.
Crigler–Najjar syndrome type 1, bilirubin glucuronides are
virtually absent in bile, whereas significant amounts of bilirubin conjugates are found in Crigler–Najjar syndrome type 2,
although the proportion of bilirubin diglucuronide is
reduced (see below). Liver biopsy is not needed for diagnosis,
unless a coexisting liver disease is suspected. If a biopsy is performed, UGT activity toward bilirubin is virtually undetectable. The diagnosis can be made also by genetic analysis
of DNA extracted from blood, buccal scrapings, or other tissue. The five exons and the flanking intronic sequences are
amplified by polymerase chain reaction and the nucleotide
sequences are determined (76). If a previously uncharacterized mutation is found, the mutation can be generated in an
expression plasmid by site-directed mutagenesis, and its effect
can be determined after transfection of the plasmid into COS
cells (47). Genetic analysis permits identification of heterozygous carriers and prenatal diagnosis based on chorionic villus
sampling or aminocentesis (93).
Animal Model
A mutant strain of Wistar rats, termed Gunn rats (94,95),
manifests nonhemolytic unconjugated hyperbilirubinemia
due to a lack of bilirubin-UGT activity. The jaundice is
inherited as an autosomal trait. The Gunn rat is the only
experimental animal that develops kernicterus spontaneously. Much of the knowledge of cellular and biochemical mechanisms of bilirubin encephalopathy has been
gained from studies on Gunn rats. The molecular basis of
UGT1A1 deficiency in this strain is the deletion of a
guanosine base in the common region exon 4. Consequently, in addition to UGT1A1, other enzymes of the
UGT1A group are also abnormal.
Treatment
Treatment is aimed at reduction of serum bilirubin levels.
Because there is hardly any residual bilirubin-UGT activity,
enzyme-inducing agents, such as phenobarbital, are ineffective in Crigler–Najjar syndrome type 1 (75). Phototherapy
is the routine treatment. An array of 140-W fluorescent
lamps is used for 8 to 12 hours a day with the eyes shielded.
After puberty, phototherapy becomes less effective because
of skin thickening, pigmentation, and decreased surface
area in relation to body mass. Phototherapy converts bilirubin IXα-ZZ into geometric and structural isomers that are
Disorders of Bilirubin Metabolism
excreted in bile without conjugation (see above). A portion
of the unconjugated bilirubin excreted in bile is reabsorbed
in the small intestine. Oral administration of agar,
cholestyramine, or calcium salts inhibits bilirubin reabsorption, thereby slightly enhancing the effect of phototherapy.
Plasmapheresis can be used to reduce serum bilirubin concentrations rapidly during crisis, although the effect is
short-lived (96). Orthotopic or auxiliary liver transplantation is the only curative therapy available at this time (97).
Because of the associated risk of liver transplantation and
the need for lifelong immunosuppression, alternative experimental therapies are being explored. Hepatocyte transplantation by infusion into the portal vein through a percutaneously placed portal venous catheter has reduced the
serum bilirubin level significantly in one patient (98,99),
but the optimum number of cells that should be transplanted for this disease is not known clearly. Immunosuppression is needed for prevention of allograft rejection.
Gene therapy methods using recombinant retrovirus, adenovirus, and SV40, as well as nonviral vectors are being
explored in studies on Gunn rats. Recently, site-directed
gene repair has been used to reduce serum bilirubin levels
in Gunn rats. These methods have been reviewed recently
(100) and are also described in Chapter 62.
Crigler–Najjar Syndrome Type 2 (Arias
Syndrome)
In this variant of Crigler–Najjar syndrome, serum bilirubin
concentrations usually range from 7 to 20 mg/dL, the prognosis is much less severe, and serum bilirubin levels are usually reduced by over 25% after administration of bilirubin-
301
UGT inducing agents, such as phenobarbital (101). Serum
bilirubin levels may be as high as 40 mg/dL during fasting
(102) or intercurrent illness (103). The bile contains significant amounts of bilirubin glucuronides (Table 20.1).
Bilirubin encephalopathy is unusual, but has been reported
(102,103). In normal bile, over 90% of the conjugated
bilirubin is bilirubin diglucuronide. In Crigler–Najjar syndrome type 2, the major pigment is bilirubin monoglucuronide (103,104). The liver has markedly reduced bilirubin-UGT activity (103).
Crigler–Najjar syndrome type 2 occurs in families (101).
There is no sex predilection. The inheritance is autosomal
recessive. As in Crigler–Najjar syndrome type I, the disease is
caused by mutations of one of the five exons that encode
bilirubin-UGT (UGT1A1) (91). However, in Crigler–Najjar
syndrome type 2, the genetic lesions are always point mutations that result in the substitution of a single amino acid
that markedly reduces, but does not abolish, bilirubin-UGT
activity (Table 20.3) (105–115). In Table 20.3, we have classified all published mutations of the UGT1A1 coding region
that result in incomplete deficiency of bilirubin glucuronidating activity as in Crigler–Najjar syndrome type 2.
Although in most of these cases serum bilirubin concentrations are clearly consistent with Crigler–Najjar syndrome
type 2, some point mutations, described in Japanese individuals, cause serum bilirubin levels that overlap with those seen
in Gilbert syndrome (see Gilbert syndrome, below). Based
on the serum bilirubin levels, some of the latter cases have
been reported in the literature by some Japanese investigators
as Gilbert syndrome (106–109,115). Such semantic difficulty in correlating genetic diagnosis with the nomenclature
that had been developed before the discovery of molecular
TABLE 20.3. MUTATIONS WITHIN THE CODING REGION OF UGT1A1 THAT REDUCE,
BUT DO NOT ABOLISH BILIRUBIN–UGT ACTIVITY
Site of Mutation
Exon
Exon
Exon
Exon
1
1
1
1/exon 5
Nucleic Acid Mutation
Predicted Amino Acid Substitution
Activity
L15R
G71R
G71R/N
G71R and Y486D
Reduced
Reduced
Reduced
Reduced
Exon 1
Exon 1
Exon 1/exon 2
T44G
G211Aa
G211A/N
Double homozygote for
G211A and T1456G
T395C
T524A
T524A/del of nt 973
L132P/N
L175Q
L175Q/truncated (frameshift)
Exon
Exon
Exon
Exon
Exon
Exon
Exon
Exon
T625C
C686A
T881C
A992G
C991T
C1099G
A1391C
T1456G
R209W
P229Q/N
I294T
Q331R
Q331X
R367G
Z464A
Y486D
Reduced activitya
Reduced activity
Reduced activity;
truncated—inactive
Reduced activity
Reduced activitya
Reduced activity
Reduced activity
Reduced activitya
Reduced activitya
Reduced activity
Reduced activity
1
1
2
2
2
4
5
5
aThese
activity
activity
activity
activitya
patients had serum bilirubin levels that overlap with the range seen in some patients with Gilbert syndrome, and
have been reported in the literature as Gilbert syndrome.
UGT, uridine-diphosphoglucuronate glucuronosyl-transferase.
Reference
105
106–108
107,108
109
108
83
83
83,111
107
88
112
113
107,108
114
107,115
302
Chapter 20
bases of these conditions is not unexpected. We propose that
reduction of UGT1A1 activity, resulting from any structural
mutation of UGT1A1, should be classified as Crigler–Najjar
syndrome type 2, and that due to a promoter abnormality
should be classified as Gilbert syndrome (see below).
Gilbert Syndrome
Gilbert syndrome, also known as “constitutional hepatic
dysfunction” or “familial nonhemolytic jaundice” (116), is
characterized by mild, chronic, and unconjugated hyperbilirubinemia (Table 20.1). Familial occurrence is common,
but not always found. The syndrome is often diagnosed in
young adults, usually males, who present with mild, predominantly unconjugated hyperbilirubinemia. Serum
bilirubin levels may fluctuate from normal to 3 mg/dL, and
increase during fasting or intercurrent illness. Occasional
patients complain of fatigue and abdominal discomfort,
which are probably manifestations of anxiety. Other than
icterus, physical examination and routine laboratory tests
are normal. Percutaneous liver biopsy, which is not required
for diagnosis, when performed, shows normal liver histology, except for a nonspecific accumulation of lipofuscin
pigment in the centrilobular zones. Hepatic bilirubin-UGT
activity is reduced to approximately 30% of normal. A
minority of patients exhibit reduced hepatic uptake of
bilirubin and other organic anions (117). Whether such
uptake defects are related pathophysiologically to Gilbert
syndrome or are merely coincidental is unknown. A 48hour fast exaggerates the unconjugated hyperbilirubinemia
of Gilbert syndrome (118). Serum bilirubin levels also
increase in normal individuals and in patients with liver diseases upon fasting. Therefore, the fasting test is of limited
diagnostic value. Intravenous injection of nicotinic acid also
increases serum bilirubin levels in Gilbert syndrome (119).
However, it does not clearly separate patients with Gilbert
syndrome from normal subjects or those with hepatobiliary
disease. As splenectomy abolishes nicotinic acid-induced
hyperbilirubinemia (119), the effect of nicotinic acid may
be based on increased erythrocyte fragility and enhanced
splenic heme oxygenase activity, leading to increased bilirubin formation.
Molecular Mechanism
The normal TATAA element within the promoter region
upstream to exon 1 of UGT1A1 has the sequence
A[TA]6TAA. A variant TATAA box, which contains a
longer dinucleotide repeat, A[TA]7TAA, has been found to
be associated with Gilbert syndrome (120). Subjects of
Caucasian, black, or Asian Indian origin, who have a clinical diagnosis of Gilbert syndrome, have been found to be
homozygous for the variant TATAA element, which reduces
the expression of the structurally normal UGT1A1. This
fits with the definition of autosomal-recessive type of inher-
itance. However, all subjects with this genotype do not
exhibit abnormally high bilirubin levels, which also depend
on other contributory factors, including the rate of bilirubin production. For example, Gilbert syndrome is diagnosed clinically much more commonly in males, although
the variant promoter is equally distributed in both genders,
probably because of a higher daily production of bilirubin
in males. Approximately 9% of the general population in
Europe and the United States are homozygous for the
Gilbert type promoter (gene frequency 0.3). The incidence
of this genotype may be lower in Japan. Some mutations in
the structural region of UGT1A1 have been reported to
result in levels of hyperbilirubinemia that are consistent
with the diagnosis of Gilbert syndrome (106–109,115).
These mutations are listed in Table 20.3 (see Crigler–Najjar
Syndrome Type 2, above).
Because of the very high incidence of the Gilbert-type
promoter, some heterozygous carriers of Crigler–Najjar syndromes type 1 or 2 mutations have the variant TATAA box
on the structurally normal allele. The consequent reduction
of expression of the only structurally normal allele can
reduce the hepatic UGT1A1 activity to a level that may
increase serum bilirubin levels to a range compatible with
the clinical diagnosis of Crigler–Najjar syndrome type 2.
This explains the frequent finding of intermediate levels of
hyperbilirubinemia in the family members of patients with
Crigler–Najjar syndrome types 1 and 2.
Although Gilbert syndrome is considered innocuous, the
diagnosis is important to avoid confusion with other liver
diseases and unnecessary investigations. Gilbert syndrome is
diagnosed in individuals with mild unconjugated hyperbilirubinemia without evidence of hemolysis or elevation of
liver enzymes. Although hemolysis is not a part of the syndrome, coexistent clinical or subclinical hemolysis may
increase the bilirubin load, thereby exacerbating the hyperbilirubinemia and bringing the patient to the attention of
the physician. When necessary, the diagnosis can be established by analysis of pigments in duodenal juice. The
reduced hepatic bilirubin-UGT activity is reflected by a
reduction of bilirubin diglucuronide to monoglucuronide
ratio in bile (104). Normally, bilirubin monoglucuronide
accounts for 10% or less of all forms of bilirubin excreted in
bile. In Gilbert syndrome the percentage increases to 14% to
34%. Genetic analysis of DNA extracted from blood leukocytes or any other tissue can aid in the diagnosis.
Animal Model
The Bolivian population of squirrel monkeys (Saimiri
siureus) has a higher serum unconjugated bilirubin levels
and a greater degree of increase upon fasting than does a
closely related Brazilian population of the species (121).
The Bolivian monkeys have slower plasma clearance of
intravenously administered bilirubin, a lower level of
hepatic bilirubin-UGT activity, and an increased bilirubin
Disorders of Bilirubin Metabolism
monoglucuronide to diglucuronide ratio in bile. In these
respects, the Bolivian squirrel monkeys are a model of
human Gilbert syndrome. Fasting hyperbilirubinemia is
rapidly reversed by oral or intravenous administration of
carbohydrates, but not by lipid administration.
DISORDERS OF BILIRUBIN METABOLISM
THAT RESULT IN PREDOMINANTLY
CONJUGATED HYPERBILIRUBINEMIA
Conjugated bilirubin may accumulate in plasma because of
“leakage” from the liver cells, as in hepatocellular diseases,
such as hepatitis, or from disordered canalicular excretion or
biliary obstruction. In all such cases, both conjugated and
unconjugated bilirubin accumulate in plasma. Rapid
advances in molecular genetic studies have revealed the
mechanism of several disorders of the hepatocyte that can,
directly or indirectly, lead to the accumulation of conjugated
bilirubin in plasma. These include Dubin–Johnson syndrome, three types of progressive intrahepatic cholestasis, and
benign recurrent intrahepatic cholestasis. Progressive familial
intrahepatic cholestasis syndromes have been discussed in
Chapter 26. The molecular basis of Rotor syndrome remains
unknown. In addition to the hepatocellular excretory abnormalities, developmental anomalies of bile ductules can cause
cholestasis. The genetic mechanism of one of these disorders,
Alagille syndrome, has been discovered.
Dubin–Johnson Syndrome
Dubin–Johnson syndrome is characterized by conjugated
hyperbilirubinemia and black pigmentation of the liver, in
303
the absence of other abnormalities of clinicochemical tests
for liver dysfunction, including serum alanine and aspartate
aminotransferase, alkaline phosphatase, γ-glutamyltranspeptidase, and albumin levels (122–124) (Table 20.4).
Dubin–Johnson syndrome is rare except in Jews of Middle
Eastern origin, in whom the incidence is 1 in 1,300 (124).
In Middle Eastern Jews, Dubin–Johnson syndrome is associated with clotting factor VII deficiency, but this linkage is
not tight. Occasionally, patients complain of vague abdominal discomfort and some have hepatosplenomegaly. In
most cases, however, the patients are asymptomatic.
Serum bile acid levels are normal and pruritus is absent
(125). Serum bilirubin levels are usually between 2 and 5
mg/dL, but may be normal at times and may be as high as
20 to 25 mg/dL during intercurrent illness, use of oral contraceptives, and pregnancy (125). Fifty percent or more of
total serum bilirubin is conjugated and bilirubinuria is frequently found. Continuous retention of bilirubin glucuronides in plasma results in the formation of irreversible
adducts of bilirubin with plasma proteins, particularly albumin (δ-bilirubin), which is not excreted in urine or bile and
gives a direct van den Bergh reaction.
Organic Anion Excretion
Canalicular excretion of many organic anions, other than
bile acids, is defective in Dubin–Johnson syndrome. These
anions include bilirubin, bromosulfophthalein (BSP),
dibromosulfophthalein (DBSP), indocyanin green (ICG),
and 125I-labeled rose Bengal. In most patients, following an
intravenous injection of BSP there is normal initial plasma
disappearance of the dye, so that the concentration is normal or mildly elevated 45 minutes after the injection. How-
TABLE 20.4. INHERITED DISORDERS CAUSING RETENTION OF BOTH
CONJUGATED AND UNCONJUGATED BILIRUBIN
Dubin–Johnson Syndrome
Serum bilirubin
Routine liver function tests
Serum bile salt levels
Plasma bromsulfophthalein
(BSP) retention
Plasma BSP clearance
Oral cholecystogram
Urinary coproporphyrin
excretion pattern
Appearance of liver
Histology of liver
Mode of inheritance
Prevalence
Prognosis
Animal model
Rotor Syndrome
Predominantly conjugated, usually 50–85 μM, can be as
high as 340 μM
Normal except for hyperbilirubinemia
Normal
Normal at 45 min; secondary rise at 90 min
Predominantly conjugated, usually 50–100
μM, occasionally as high as 340 μM
Normal except for hyperbilirubinemia
Normal
Elevated; but no secondary rise at 90 min
Tmax is very low; storage is normal
Usually does not visualize the gallbladder
Total—normal; >80% as coproporphyrin I
Both Tmax and storage are reduced
Usually visualizes the gallbladder
Total—elevated; ~50–75% coproporphyrin I
Grossly black
Dark pigments, predominantly in centrilobular areas;
otherwise normal
Autosomal recessive
Rare (except in Middle Eastern Jews: 1 in 1,300 births)
Benign
Mutant TR− rats/mutant Corriedale
sheep/golden lion Tamarin monkey
Normal
Normal, no increase in pigmentation
Autosomal recessive
Rare
Benign
None
304
Chapter 20
ever, 90 minutes after the injection, there is a secondary rise
because of the reflux of glutathione-conjugated BSP from
the liver cell into the circulation prior to excretion by the
hepatocytes (126,127). A similar secondary rise has been
described following intravenous administration of unconjugated bilirubin. However, such secondary rise can also
occur in other cholestatic disorders. Because of the organic
anion excretion defect, oral cholecystographic contrast dyes
do not visualize the gallbladder even after a double dose.
Hepatic Pigmentation
Macroscopically, the liver is black. Liver histology is normal
except for the accumulation of a dense pigment, which is
contained within lysosomes (128). Infusion of 3H-epinephrine in the Corriedale sheep (an animal model of
Dubin–Johnson syndrome, see below) revealed reduced biliary excretion of radioactivity and incorporation of the isotope into the hepatic pigment, suggesting its relationship
with melanin (129). When TR− rats (another model of
Dubin–Johnson syndrome) are fed a diet enriched in aromatic amino acids (phenylalanine, tyrosine, and tryptophan), lysosomal pigmentation develops, probably because
of impaired excretion of anionic metabolites of tyrosine,
phenylalanine, and tryptophan, with subsequent oxidation,
polymerization, and lysosomal accumulation (130). Electron spin resonance spectroscopy suggests that the pigment
differs from authentic melanin, but could be composed of
polymers of epinephrine metabolites. Computed tomography of the liver shows higher than normal attenuation values in Dubin–Johnson syndrome. Interestingly, the pigment is cleared during acute viral hepatitis and
reaccumulates slowly after recovery (131).
Molecular Mechanism
Organic anions, other than bile acids, such as conjugated
bilirubin, and other glucuronide or glutathione conjugated
substances, are transported across the bile canalicular membrane by an ATP-dependent energy-consuming process,
mediated by MRP2 [also known as the canalicular multispecific organic anion transporter (cMOAT)] (Fig. 20.5)
(see Chapters 24 and 25). TR− rats have a frame-shift mutation in the gene encoding MRP2 (134). The human MRP2
gene is located on chromosome 10q23-q24. A number of
mutations causing Dubin–Johnson syndrome have been
identified, a significant proportion of which are in the critical ATP-binding domain (135–139) (Table 20.5). A mutation at an intronic splice donor site that results in abnormal
splicing of the transcript has also been identified in a
patient with Dubin–Johnson syndrome (139).
Animal Models
A mutant strain of the Corriedale sheep was found to have
a metabolic defect similar to that in Dubin–Johnson syndrome. Biliary excretion of conjugated bilirubin, glutathione-conjugated BSP, iopanoic acid, and ICG is
decreased in this strain, whereas taurocholate transport is
normal. The secretion of unconjugated BSP is unimpaired.
As in patients with Dubin–Johnson syndrome, total urinary
coproporhyrin excretion is normal with increased proportion of the isomer I. The most extensively studied animal
model for Dubin–Johnson syndrome is the TR− rat (140).
The organic anion excretion defect and the pattern of
Urinary Coproporphyrin Excretion
The total urinary coproporphyrin excretion is normal in
Dubin–Johnson syndrome, but the ratio of coproporphyrin I to coproporphyrin III is greater (4:1), than that
seen normally (1:3) (132). In obligate heterozygotes (i.e.,
unaffected parents and children of patients with
Dubin–Johnson syndrome), total urinary coproporphyrin
excretion is reduced by 40%, because of a 50% reduction
in coproporphyrin III excretion (133). In heterozygote
carriers, the proportion of coproporphyrin I in urine was
intermediate between findings in controls and in patients
with Dubin–Johnson syndrome. Based on these data,
Dubin–Johnson syndrome is inherited as an autosomalrecessive characteristic. No other hepatobiliary disorder or
porphyria has been described in which a combination of
normal total urinary coproporphyrin excretion and a great
predominance of coproporphyrin I is seen. Thus, in the
presence of a consistent history and physical examination,
urinary coproporphyrin excretion appears to be diagnostic
of this disorder.
FIGURE 20.5. Four adenosine triphosphate–utilizing transport
proteins concentrated in the bile canalicular membrane have
been recognized to be important in canalicular transport. Multidrug resistance-related protein (MRP2) [also known as canalicular multispecific organic anion transporter (cMOAT)] mediates
the transport of most non–bile-acid organic anions, including
bilirubin glucuronides. Bile salt export pump (BSEP) [also known
as sister of p-glycoprotein (SPGP)] is the major bile acid transporter. FIC1 translocates acidic phospholipids (such as phosphatidylserine and phosphatidyl-ethanolamine) from the outer
to the inner leaf of the plasma membrane. MDR3 transports
phospholipids from the inner to the outer leaflet of the bile
canaliculus. Genetic lesions of MRP2 cause Dubin–Johnson syndrome. Inherited abnormalities of the other three genes are
associated with various intrahepatic cholestasis syndromes (see
text). FIC, familial intrahepatic cholestasis; MDR, multi drug resistance.
Disorders of Bilirubin Metabolism
305
TABLE 20.5. MUTATIONS IDENTIFIED IN PATIENTS WITH DUBIN–JOHNSON SYNDROME TYPE
Site of Mutation
Nucleic Acid Change
Predicted Change of Amino Acid in MRP2
Reference
Exon 13
Intron 15
Exon 18
Exon 18
Exon 23
Exon 31
Del, nt 1669–1815
Splice donor site, T→C
C2302T
Del, nt 2272–2439
C3196T
Del, nt 4175–4180
Truncated protein
Truncated protein
R368W
Truncated protein
R1066X—truncated protein
Truncated protein
138
139
138
138
137
135
MRP, multidrug resistance-related protein.
coproporphyrin excretion in urine are similar to that in
Dubin–Johnson syndrome. For organic anions, such as glutathione-conjugated leukotriene (LT)C4, the canalicular
secretion defect is nearly complete, whereas for bilirubin
glucuronides there is about 10% residual transport activity
(141). The TR− rat and patients with Dubin–Johnson syndrome have normal canalicular excretion of bile salts, except
those that have double-negative charges because of conjugation at the 3-OH position (142). The ATP-driven component of bilirubin glucuronide transport by canalicular
plasma membrane vesicles is absent in the TR− rats, but the
membrane potential-dependent mechanism provides the
residual transport (53). A mutant strain of golden lion
tamarins (Leontopitheous rosalia rosalia) with Dubin–Johnson-like syndrome has been described (143).
Rotor Syndrome
This disorder is characterized by accumulation of conjugated bilirubin in the plasma in the presence of normal liver
function tests (144) (Table 20.4). In contrast to Dubin–
Johnson syndrome, there is no increased pigmentation of
the liver. Oral cholecystographic agents result in roentgenologic visualization of the gallbladder in Rotor syndrome.
Unlike the findings in Dubin–Johnson syndrome, patients
with Rotor syndrome exhibit marked retention of BSP at
45 minutes after injection, but biphasic plasma BSP peaks
are not found and conjugated BSP does not appear in
plasma. There is also marked plasma retention of intravenously administered unconjugated bilirubin and ICG.
Studies using a constant infusion of BSP indicate that
while in Dubin–Johnson syndrome the transport maximum (Tmax) is virtually zero and hepatic storage is normal,
in Rotor syndrome the Tmax is 50% of normal, but the
hepatic storage is reduced by 75% to 90%. Thus,
Dubin–Johnson syndrome represents a canalicular excretion disorder, whereas Rotor syndrome is a disorder of
hepatic storage and may be identical with the so-called
familial hepatic storage disease (145).
Urinary Coproporphyrin Excretion
Compared to normal, total urinary coproporphyrin excretion is increased by 250% to 500% and the proportion of
coproporphyrin I in urine is approximately 65% of total
(146). These results are similar to those seen in many other
hepatobiliary disorders and distinguish this disorder from
Dubin–Johnson syndrome. Rotor syndrome is inherited as
an autosomal-recessive characteristic. Its molecular basis is
unknown.
Progressive Familial Intrahepatic
Cholestasis Syndromes
In contrast to Dubin–Johnson and Rotor syndromes, progressive familial intrahepatic cholestasis syndromes (PFICs)
are autosomal-recessive disorders, associated with various
degrees of cholestasis. In most cases PFICs cause progressive
liver damage. An exception is benign recurrent intrahepatic
cholestasis, which is an episodic and milder disorder. These
conditions have been discussed in Chapter 26.
Alagille Syndrome
Several inherited disorders of bile duct development have
been described. Of these, the Alagille syndrome was the first
to be characterized at the molecular level. Alagille syndrome
is characterized by the paucity or absence of small bile
ducts, resulting in progressive intrahepatic cholestasis, and
abnormalities of the eye, heart, and vertebrae. The disorder
is inherited as an autosomal-dominant characteristic. The
responsible gene, JAG1, has been mapped to chromosome
20p12 (147). JAG1 encodes an unidentified ligand that
binds to the notch receptor, which is crucial for cell plate
development in Drosophila and mammals. In rare cases, the
gene is deleted. In other cases of Alagille syndrome, various
point mutations in JAG1, each of which abolishes expression of the altered allele, have been described.
ACKNOWLEDGMENTS
The authors thank Dr. Ajit Kadakol for assistance in preparation of this review. This work was supported in part by
National Institutes of Health grants DK-46057, DK-39137,
DK-41296, DK-23026, DK-35652, and DK-34926.
306
Chapter 20
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The Liver: Biology and Pathobiology, Fourth Edition, edited by I. M. Arias, J. L. Boyer, F. V. Chisari, N. Fausto, D. Schachter, and D. A. Shafritz.
Lippincott Williams & Wilkins, Philadelphia © 2001.